Purpose: Heart rate disorders are responsible for ventricular remodeling and enhanced susceptibility to cardiac arrhythmias. In experimental bradycardia electrical remodeling of cardiac myocytes (CM) includes a reduction of the delayed rectifier K + currents, which are responsible for action potential repolarization delay and increased propensity to develop potentially lethal arrhythmias. The aim of this study was to evaluate ventricular remodeling occurring in a novel model of bradycardia (Baruscotti M., PNAS 2011), based on inducible and cardiac specific ablation of HCN4 gene encoding for the f current in sinoatrial node cells. Methods: Cardiac HCN4 knockout was induced by i.p. injections of tamoxifen (200 mg/Kg) for 5 consecutive days in adult HCN4lox/lox;Cre mice. Control mice underwent the same treatment. Heart rate was monitored daily. Electrophysiological study was performed using the single-cell patch-clamp technique. Gene expression was studied by quantitative RT-PCR on ventricular tissue. Results: Tamoxifen injections produced a progressive development of bradycardia that reduced heart rate by 25% in the HCN4lox/lox;Cre mice but not in control animals. Bradycardia was associated to 75% reduction of cardiac HCN4 mRNA level. Patch-clamp recordings on ventricular CM showed a marked prolongation of action potential duration in HCN4lox/lox;Cre bradycardic mice with respect to control animals (80+0.4 vs 30+0.1 ms at 90% of repolarization). Quantitative mRNA expression of subunits underlying repolarizing currents showed downregulation of the inward-rectifier K + channel subunit Kir2.1 (-60%), the slow delayed-rectifier K + channel subunit Kcnq1 (-50%), and the transient outward K + channel subunits Kv4.2 (-80%),Kv4.3 (-50%) and KChIP2 (-90%) in HCN4lox/lox;Cre bradycardic mice with respect to control animals. The rapid delayed-rectifier K + channel subunit erg and the regulatory subunit MinK were unchanged, while the regulatory subunit Mirp-1 was upregulated. Conclusions: The HCN4lox/lox;Cre transgenic mouse represents an innovative and reliable model of inducible bradycardia useful to study rate-related electrical remodeling of CM. In accordance to different model (Gross GJ, J Cardiovasc Electrophysiol 2006), we identified a prominent repolarization delay of ventricular action potential as major electrophysiological modification in bradycardic HCN4lox/lox;Cre mice. Expression studies point to a crucial role for the downregulation of the inward-rectifier, the slow delayed-rectifier, and the transient outward K + channels to underlie electrical remodeling in braycardic HCN4lox/lox;Cre mice.
Ventricular remodeling in a murine model of cardiac selective and inducible deletion of HCN4 gene / M. Del Lungo, L. Sartiani, V. Spinelli, M. Baruscotti, D. Difrancesco, A. Mugelli, E. Cerbai. - In: CARDIOVASCULAR RESEARCH. - ISSN 0008-6363. - 93:Suppl. 1(2012), pp. S65-S65. ((Intervento presentato al 2. convegno Congress of the European Society of Cardiology - Council on Basic Cardiovascular Science - Frontiers in cardiovascular biology tenutosi a London nel 2012.
Ventricular remodeling in a murine model of cardiac selective and inducible deletion of HCN4 gene
M. Baruscotti;D. Difrancesco;
2012
Abstract
Purpose: Heart rate disorders are responsible for ventricular remodeling and enhanced susceptibility to cardiac arrhythmias. In experimental bradycardia electrical remodeling of cardiac myocytes (CM) includes a reduction of the delayed rectifier K + currents, which are responsible for action potential repolarization delay and increased propensity to develop potentially lethal arrhythmias. The aim of this study was to evaluate ventricular remodeling occurring in a novel model of bradycardia (Baruscotti M., PNAS 2011), based on inducible and cardiac specific ablation of HCN4 gene encoding for the f current in sinoatrial node cells. Methods: Cardiac HCN4 knockout was induced by i.p. injections of tamoxifen (200 mg/Kg) for 5 consecutive days in adult HCN4lox/lox;Cre mice. Control mice underwent the same treatment. Heart rate was monitored daily. Electrophysiological study was performed using the single-cell patch-clamp technique. Gene expression was studied by quantitative RT-PCR on ventricular tissue. Results: Tamoxifen injections produced a progressive development of bradycardia that reduced heart rate by 25% in the HCN4lox/lox;Cre mice but not in control animals. Bradycardia was associated to 75% reduction of cardiac HCN4 mRNA level. Patch-clamp recordings on ventricular CM showed a marked prolongation of action potential duration in HCN4lox/lox;Cre bradycardic mice with respect to control animals (80+0.4 vs 30+0.1 ms at 90% of repolarization). Quantitative mRNA expression of subunits underlying repolarizing currents showed downregulation of the inward-rectifier K + channel subunit Kir2.1 (-60%), the slow delayed-rectifier K + channel subunit Kcnq1 (-50%), and the transient outward K + channel subunits Kv4.2 (-80%),Kv4.3 (-50%) and KChIP2 (-90%) in HCN4lox/lox;Cre bradycardic mice with respect to control animals. The rapid delayed-rectifier K + channel subunit erg and the regulatory subunit MinK were unchanged, while the regulatory subunit Mirp-1 was upregulated. Conclusions: The HCN4lox/lox;Cre transgenic mouse represents an innovative and reliable model of inducible bradycardia useful to study rate-related electrical remodeling of CM. In accordance to different model (Gross GJ, J Cardiovasc Electrophysiol 2006), we identified a prominent repolarization delay of ventricular action potential as major electrophysiological modification in bradycardic HCN4lox/lox;Cre mice. Expression studies point to a crucial role for the downregulation of the inward-rectifier, the slow delayed-rectifier, and the transient outward K + channels to underlie electrical remodeling in braycardic HCN4lox/lox;Cre mice.
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